First published February 1, 2010Submitted: August 27,
2009; Accepted: December 9,
2009.

Diet-induced obesity (DIO) leads to inflammatory activation of macrophages in white adipose tissue (WAT) and subsequently to insulin resistance. PPARγ agonists are antidiabetic agents known to suppress inflammatory macrophage activation and to induce expression of the triacylglycerol (TG) synthesis enzyme acyl CoA:diacylglycerol acyltransferase 1 (DGAT1) in WAT and in adipocytes. Here, we investigated in mice the relationship between macrophage lipid storage capacity and DIO-associated inflammatory macrophage activation. Mice overexpressing DGAT1 in both macrophages and adipocytes (referred to herein as aP2-Dgat1 mice) were more prone to DIO but were protected against inflammatory macrophage activation, macrophage accumulation in WAT, systemic inflammation, and insulin resistance. To assess the contribution of macrophage DGAT1 expression to this phenotype, we transplanted wild-type mice with aP2-Dgat1 BM. These mice developed DIO similar to that of control mice but retained the protection from WAT inflammation and insulin resistance seen in aP2-Dgat1 mice. In isolated macrophages, Dgat1 mRNA levels correlated directly with TG storage capacity and inversely with inflammatory activation by saturated fatty acids (FAs). Moreover, PPARγ agonists increased macrophage Dgat1 mRNA levels, and the protective effects of these agonists against FA-induced inflammatory macrophage activation were absent in macrophages isolated from Dgat1-null mice. Thus, increasing DGAT1 expression in murine macrophages increases their capacity for TG storage, protects against FA-induced inflammatory activation, and is sufficient to reduce the inflammatory and metabolic consequences of DIO.

Introduction

Chronic diet-induced obesity (DIO) promotes infiltration of the white adipose tissue (WAT) by monocyte-derived phagocytic and antigen-presenting cells that include macrophages and dendritic cells. These macrophages accumulate in crown-like structures (CLS) around dying or apoptotic adipocytes and change their overall polarity from a relatively antiinflammatory (M2) activation state to a more inflammatory (M1) state (1–5). The M1 activation of macrophages in WAT is linked to chronically elevated serum levels of inflammatory cytokines, such as TNF-α, that are key to the development of insulin resistance, diabetes, and atherosclerosis (6–9).

Determining the molecular mechanisms that trigger M1 activation of macrophages in WAT during DIO may offer insights into the metabolic consequences of obesity. Recent evidence points to the importance of saturated fatty acids (FAs), which are systemically elevated in chronic DIO (10, 11) and stimulate M1 activation of macrophages and dendritic cells in culture (12–15). This stimulation is mediated, at least in part, by signaling through TLR2 and TLR4 and the associated activation of JNK (13–17). However, M1 activation may also be influenced by the levels of intracellular FAs, which regulate a wide variety of signaling pathways (18–22). These intracellular FAs exist in different pools, including free FAs, FA acyl CoAs, and inert FA moieties that are incorporated into glycerolipids, such as triacylglycerols (TGs) (23). The capacity of macrophages to incorporate FAs into TGs could thus serve to modulate the potential for M1 activation.

Synthesis of TG involves acyl CoA:diacylglycerol acyltransferase (DGAT) enzymes, which catalyze a reaction with diacylglycerol and FA acyl CoA substrates (23). Cellular TG storage is directly correlated with levels of DGAT activity. For example, overexpression of DGAT enzymes in transgenic mice is sufficient to increase cellular TG storage in WAT, skeletal muscle, or liver in a tissue-specific manner (24–26). Moreover, DGAT1 helps to protect cultured cells from the toxic effects of excess FAs (27). Interestingly, DGAT1 expression in adipocytes and WAT is upregulated by PPARγ activation (28–30), and PPARγ activation protects macrophages against M1 activation in vitro and in vivo (13, 31–33). Given these findings, we hypothesized that DGAT1 expression in macrophages may modulate M1 activation by FAs.

In the current study, we examined this hypothesis by performing a series of studies in genetically modified mice to determine how increasing DGAT1 expression in the macrophage compartment affects the response to a chronically high-fat diet. We also examined primary macrophages from genetically modified mice to determine whether the level of DGAT1 expression modulates FA- and cytokine-induced M1 activation in a cell-autonomous manner. Finally, we determined whether DGAT1 is regulated by PPARγ agonists in macrophages and whether DGAT1 is required for the antiinflammatory effects of PPARγ agonists on FA-induced M1 activation.

Results

aP2-Dgat1 mice have increased Dgat1 mRNA levels in both adipocytes and macrophages. We previously showed that transgenic C57BL/6 mice overexpressing murine Dgat1 under the control of the FA-binding protein 4 (aP2) promoter (aP2-Dgat1) have increased Dgat1 mRNA levels in WAT (24). However, the aP2 promoter can drive gene expression in both adipocytes and monocyte-derived macrophages and dendritic cells (34, 35). We therefore examined the contribution of these cell types to increased Dgat1 mRNA levels in aP2-Dgat1 WAT. We harvested the epididymal fat pads from mice, keeping 1 fat pad intact and separating the other to yield adipocytes and a macrophage-containing stromal-vascular fraction (SVF). We then analyzed mRNA levels in the whole WAT, adipocytes, and SVF by quantitative PCR (qPCR) (Figure 1A). Dgat2 mRNA was highly expressed specifically in adipocytes, a cell type rich in DGAT2, while Emr1 (EGF-like module-containing mucin-like receptor 1 or F4/80), a macrophage-expressed gene, was highly expressed in the SVF, verifying the integrity of the adipocyte and macrophage fractions. Although Dgat1 mRNA levels were, as expected, increased (~10-fold) in the whole WAT of aP2-Dgat1 mice, this increase occurred to a similar magnitude in adipocytes and the SVF, suggesting that the transgene is expressed in both adipocytes and monocyte-derived macrophages.

To assess DGAT1 overexpression specifically in macrophages, we measured Dgat1 mRNA levels in peritoneal macrophages (P-Mϕ) and BM-derived macrophages (BMD-Mϕ) from aP2-Dgat1 mice. Whereas the mRNA levels of controls Dgat2 and Emr1 were similar in WT and aP2-Dgat1 mice, Dgat1 mRNA levels were increased (~6–8.5-fold) in the P-Mϕ of aP2-Dgat1 mice whether they were fed a chow diet or a 16-week high-fat diet (Figure 1B). Interestingly, mRNA levels of both Dgat1 and Dgat2 were increased dramatically (~50-fold for Dgat1 and ~800-fold for Dgat2) in macrophages after high-fat feeding in WT mice (Figure 1B), suggesting both enzymes are involved in the response of macrophages to a high-fat diet. For Dgat1, the increase was further accentuated in the transgenic mice such that mRNA levels were over 200-fold higher than baseline levels. Dgat1 mRNA levels were also increased in BMD-Mϕ from aP2-Dgat1 mice (Figure 1C), as were DGAT1 protein levels (Figure 1D).

aP2-Dgat1 mice are prone to accentuated DIO but protected against its metabolic and inflammatory consequences. To determine the impact of increased Dgat1 mRNA levels in the adipocyte/macrophage compartment on obesity and diet-induced insulin resistance, WT and aP2-Dgat1 mice were fed a chow diet or a high-fat diet for 16 weeks. On either diet, aP2-Dgat1 mice gained more weight than WT mice (Figure 2A), and an analysis of body composition by dual energy X-ray absorptiometry (DEXA) showed increased adiposity (Figure 2B). Glucose tolerance was similar in aP2-Dgat1 and WT mice fed a chow diet (data not shown). However, despite their relative obesity, aP2-Dgat1 mice chronically fed a high-fat diet had less TG accumulation in the skeletal muscle and liver (Figure 2C) and enhanced glucose and insulin tolerance (Figure 2D). aP2-Dgat1 mice with chronic DIO also had lower fasting levels of insulin and glucose and a lower mean value on the homeostasis model assessment of insulin resistance (HOMA-IR) index, indicative of improved insulin sensitivity (Table 1). aP2-Dgat1 mice with chronic DIO displayed other phenotypic features associated with enhanced insulin sensitivity. Serum resistin levels, which increase with DIO and promote insulin resistance (36), were not elevated in aP2-Dgat1 mice, and serum adiponectin levels, which correlate inversely with the degree of DIO and insulin resistance (37), were higher in aP2-Dgat1 mice (Table 1). Additionally, aP2-Dgat1 mice had lower serum TG levels when fed a high-fat diet (Table 1), as reported (24).

Given their improvement in insulin and glucose metabolism, we hypothesized that the aP2-Dgat1 mice would have less diet-induced inflammation in the WAT. In agreement with this, the expression of genes induced by M1 macrophage activation, including Nos2 (iNOS), Itgax (integrin, alpha X [complement component 3 receptor 4 subunit] or CD11c), and those encoding for inflammatory cytokines (Tnfa), and chemokines (Ccl2, or monocyte chemoattractant protein-1 [MCP-1]), were reduced in the WAT of aP2-Dgat1 mice chronically fed a high-fat diet (Figure 3A). In contrast, mRNA levels for genes marking the alternative (M2) activation state of macrophages were not different between genotypes (Figure 3A). Taken together, these data indicate that aP2-Dgat1 mice chronically fed a high-fat diet have reduced activation of the M1 inflammatory pathway in the WAT.

Activated resident WAT macrophages promote inflammation by recruiting more macrophages, which accumulate in CLS around adipocytes on histological sections (1–5). The number of such structures in WAT was reduced by more than 50% in high-fat–fed aP2-Dgat1 mice (Figure 3B). Thus, DIO in aP2-Dgat1 mice is associated with reductions in both the M1 activation and accumulation of macrophages in the WAT, 2 components of chronic WAT inflammation. These differences were not seen in chow-fed mice, in which CLS were rarely seen in WAT (data not shown). Consistent with decreased recruitment of macrophages into the WAT, we found that aP2-Dgat1 mice had 20%–40% lower levels of the serum proinflammatory factors TNF-α, MCP-1, and plasminogen activator inhibitor-1 (PAI-1) (Figure 3C).

Protection against inflammatory and metabolic consequences of DIO in aP2-Dgat1 mice does not require adiponectin. The WAT-derived hormone adiponectin modulates metabolic and inflammatory parameters in mice (29, 38–42). Because aP2-Dgat1 mice had 60% more serum adiponectin (Table 1), adiponectin emerged as a potential contributor to the phenotype of aP2-Dgat1 mice. To address this possibility, we crossed aP2-Dgat1 mice with adiponectin-deficient (Adipoq–/–) mice (39) to generate Adipoq–/–aP2-Dgat1 mice and examined the inflammatory and metabolic responses of these mice to chronic DIO. On a chow diet, Adipoq–/–aP2-Dgat1 mice gained slightly more weight than Adipoq–/– mice (Supplemental Figure 1A; supplemental material available online with this article; doi:
10.1172/JCI36066DS1). However, when fed a 16-week high-fat diet, the weight curves of Adipoq–/– mice, which are prone to DIO (39), and Adipoq–/–aP2-Dgat1 mice were similar (Supplemental Figure 1A), suggesting an epistatic interaction of these alleles in this dietary condition.

As expected, Adipoq–/– mice developed diet-induced glucose intolerance (Supplemental Figure 1B). Remarkably, however, Adipoq–/–aP2-Dgat1 had improved glucose tolerance and lower fasting insulin levels on a high-fat diet than did Adipoq–/– mice (Supplemental Figure 1B and Supplemental Table 1), indicating that overexpression of DGAT1 in the adipocyte/macrophage compartment was sufficient to suppress the impairment in glucose metabolism induced by adiponectin deficiency. Further, Adipoq–/–aP2-Dgat1 mice with chronic DIO had lower mRNA levels of M1 macrophage genes in the WAT (Supplemental Figure 1C) and lower serum levels of TNF-α, MCP-1, and PAI-1 (Supplemental Figure 1D) than did Adipoq–/– mice. TG levels in the serum (Table 1) and in the livers and skeletal muscle (Supplemental Figure 1E) were also lower in Adipoq–/–aP2-Dgat1 mice with DIO. These results indicate that the protective metabolic effects of DGAT1 overexpression in aP2-Dgat1 mice with DIO are independent of adiponectin.

BM transplantation to generate mice with overexpression of DGAT1 in macrophages. Our studies of aP2-Dgat1 transgenic mice indicated that the overexpression of DGAT1 in the adipocyte/macrophage compartment yielded metabolic benefits in the setting of DIO but could not distinguish the relative contributions of adipocytes and macrophages to this effect. Because of the concomitantly reduced inflammatory state of aP2-Dgat1 mice, we elected to further study the effects of DGAT1 overexpression in monocyte-derived macrophages. To this end, we transplanted lethally irradiated WT mice with BM from age-matched WT or aP2-Dgat1 mice. Our experimental design (Figure 4A) yielded one cohort of mice in which both macrophages and adipocytes were genetically WT (WT→WT) and another in which Dgat1 mRNA levels were increased in macrophages but not in adipocytes (Tg→WT). By using donor marrow (CD45.2) and recipient marrow (CD45.1) that were genetically identical except for a single point mutation, we confirmed that 94%–98% of peripheral leukocytes in transplanted mice were of donor origin 1 month after the procedure (Figure 4B).

Complete and specific reconstitution in mice transplanted with WT or aP2-Dgat1 BM.
(A) Depiction of the Dgat1 genotype expected in adipocytes and macrophages of WT mice transplanted with either WT or aP2-Dgat1 BM. (B) Representative FACS plots of peripheral blood leukocytes from mice, performed with FITC-coupled anti-CD45.1 and APC-coupled anti-CD45.2 antibodies, showing recipient (CD45.1-positive) and donor (CD45.2-positive) cells (top) and that more than 94% of leukocytes after transplant were of donor origin. (C) Expression of the aP2-Dgat1 transgene is detectable in blood of recipients of Tg→WT donors but not WT→WT controls. PCR was performed with aP2-Dgat1–specific primers. Tail DNA from known aP2-Dgat1 mice. C indicates a positive control for the transgene. (D) Increased Dgat1 mRNA levels specifically in the SVF of Tg→WT mice. mRNA levels were measured by qPCR from the livers and whole and fractionated WAT of transplanted mice (n = 7–13 per group) fed a high-fat diet for 20 weeks (*P < 0.05).

To detect aP2-Dgat1 cells in the blood of Tg→WT mice, we performed PCR on genomic DNA from whole-blood samples with primers unique to the aP2-Dgat1 transgene. The aP2-Dgat1 amplification product was not found in samples from WT→WT mice but was present in each of the samples from Tg→WT mice, indicating the reconstitution of blood with aP2-Dgat1 leukocytes in Tg→WT mice (Figure 4C).

To determine which compartments of the WAT were reconstituted by transplantation, we analyzed Dgat1 mRNA levels in both whole and fractionated WAT. The mRNA levels of the control genes Dgat2 and Emr1 in each WAT compartment were similar between groups (Figure 4D). However, the Dgat1 mRNA levels of Tg→WT mice were selectively increased in the SVF and not in the whole WAT or adipocytes (Figure 4D). Taken together, these data are consistent with Tg→WT mice having increased Dgat1 mRNA levels in circulating monocytes and WAT macrophages but not in adipocytes.

Increased Dgat1 expression in macrophages is sufficient to protect mice against diet-induced insulin resistance. To determine the metabolic impact of increasing DGAT1 expression in monocyte-derived macrophages, WT→WT and Tg→WT mice were fed a high-fat diet for 16 weeks. Both groups of transplanted mice developed a similar level of moderate DIO (Figure 5A). Although this DIO was less marked than that induced in nontransplanted mice (see Figure 2A), both groups of transplanted mice gained weight at a rate greater than that of nontransplanted WT mice fed a chow diet (see Figure 2A) and similar to that in another report of transplanted C57BL/6 mice fed a high-fat diet (43). Unlike aP2-Dgat1 mice, Tg→WT mice were not protected against diet-induced nonadipose tissue steatosis (Figure 5B). Remarkably, however, Tg→WT mice with DIO exhibited enhanced glucose and insulin tolerance, indicating that the transfer of hematopoietic cells with increased DGAT1 expression is sufficient to protect mice against diet-induced alterations in glucose metabolism (Figure 5C).

Increased Dgat1 expression in macrophages is sufficient to protect mice against inflammatory consequences of DIO. We next determined whether Tg→WT mice were protected against the inflammatory consequences of obesity. The mRNA levels of M1 macrophage genes were reduced in the WAT of Tg→WT mice fed a high-fat diet for 20 weeks (Figure 6A), and separation of the WAT revealed a corresponding reduction in the mRNA levels of these genes in the SVF but not in the adipocytes. These findings indicate that transfer of hematopoietic cells with increased Dgat1 mRNA levels is sufficient to protect mice against diet-induced M1 macrophage activation in the WAT. The mRNA levels of M2 genes were similar in WT→WT and Tg→WT mice with chronic DIO, indicating that the protection against macrophage activation in the WAT of Tg→WT mice was specific to the M1 pathway (Figure 6B). Consistent with this, WAT sections from Tg→WT mice showed fewer macrophage CLS (Figure 6C), indicating that these mice were protected against the diet-induced accumulation of macrophages in the WAT. The only cytokine with serum levels sufficient for accurate measurement was PAI-1, and these levels were 3-fold lower in Tg→WT mice than in WT→WT mice (491 ± 199 versus 1530 ± 358 pg/ml; n = 6–10 per group; P < 0.05).

Transplantation of aP2-Dgat1 BM is sufficient to protect mice against diet-induced inflammation in WAT.
(A) Lower mRNA levels of M1 pathway genes specifically in the whole WAT and SVF of Tg→WT mice. (B) Similar mRNA levels of M2 pathway genes in the whole WAT and SVF of Tg→WT and WT→WT mice. For A and B, mRNA levels were measured by qPCR in whole and fractionated WAT from transplanted mice fed a high-fat diet for 20 weeks (n = 7–13 per group; *P < 0.05). (C) Fewer CLS in the WAT of Tg→WT mice (n = 4-5 mice per group). Macrophages from WAT sections were stained with anti-F4/80 (top), and quantified from serial sections at bottom (*P < 0.01). Scale bars: 50 μM.

Dgat1 mRNA levels in cultured macrophages determine TG storage capacity. Our studies in Tg→WT mice showed that increasing DGAT1 expression in macrophages had a profound effect on the M1 activation of WAT macrophages associated with DIO. To determine whether these effects could be extended in vitro, we cultured BMD-Mϕ from mice with different levels of DGAT1 expression and treated these cells with monounsaturated oleic acid and saturated palmitic acid, 2 abundant dietary FAs. In particular, treatment of cultured macrophages with palmitate activates the M1 response (12–15).

We first assessed the ability of BMD-Mϕ to store FAs as TGs. WT macrophages were incubated with radiolabeled oleate or palmitate for 24 hours to enable examination of FA flux. Both oleate and palmitate were taken up by cells and similarly incorporated into the cellular lipid pool (Figure 7A). However, whereas half of the radiolabeled oleate taken up by cells was incorporated into TG, only approximately 12% of the palmitate was present in this fraction, indicating a preference by WT cells for esterifying oleate (Figure 7A).

We next determined whether changes in Dgat1 mRNA levels altered TG storage capacity in BMD-Mϕ. Incubation of WT and aP2-Dgat1 BMD-Mϕ with oleate showed that macrophages with increased DGAT1 expression had larger and more numerous lipid droplets (Figure 7B). The analysis of BMD-Mϕ from Dgat1-deficient (Dgat1–/–), WT, and aP2-Dgat1 mice incubated with FAs for 24 hours showed that the level of Dgat1 expression correlated directly with neutral lipid content (Figure 7C). In fact, aP2-Dgat1 BMD-Mϕ in medium without added FA (control) had a higher neutral lipid content than WT or Dgat1–/– cells. Oleate treatment did not increase the neutral lipid content of Dgat1–/– cells, but did so for both WT and aP2-Dgat1 cells in a stepwise manner correlating with Dgat1 mRNA level. Furthermore, although palmitate treatment did not increase the neutral lipid content of WT cells (by this method or by TLC) or Dgat1–/– cells, it did so for aP2-Dgat1 cells. Thus, the level of Dgat1 mRNA in BMD-Mϕ directly correlates with their capacity for TG storage whether treated with oleate or palmitate.

The level of Dgat1 expression modulates M1 inflammatory activation in BMD-Mϕ. Inasmuch as DGAT1 expression levels affected TG storage capacity in macrophages, we hypothesized that expression levels would also modulate their vulnerability to M1 inflammatory activation in response to FAs. Culturing WT BMD-Mϕ with palmitate but not oleate activated the M1 pathway (Figure 8A). We therefore tested to determine whether the level of Dgat1 mRNA expressed in BMD-Mϕ affects the M1 response to palmitate treatment. In untreated (control) cells, the expression of M1 genes was relatively low and varied little between DGAT1 genotypes, although Dgat1–/– cells had increased mRNA levels of Nos2 and aP2-Dgat1 cells had decreased levels of Tnfa (Figure 8B). In cells treated with palmitate for 24 hours, mRNA levels of all M1 markers were increased in WT BMD-Mϕ, and levels of Tnfa and Nos2 were increased relatively more in Dgat1–/– cells. In contrast, mRNA levels of all M1 markers were decreased in palmitate-treated aP2-Dgat1 BMD-Mϕ, indicating an inverse correlation between the levels of Dgat1 mRNA in BMD-Mϕ and the induction of M1 gene expression by palmitate treatment.

M1-type activated macrophages secrete more IL-6, MCP-1, and TNF-α (1, 13, 14). We therefore measured the levels of these cytokines in the medium of Dgat1–/–, WT, and aP2-Dgat1 BMD-Mϕ treated with palmitate. In untreated controls, cytokine levels were relatively low, and medium from Dgat1–/– cells had slightly higher MCP-1 levels than medium from WT and aP2-Dgat1 BMD-Mϕ (Figure 8C). Palmitate treatment increased the levels of each cytokine in the medium from BMD-Mϕ of each genotype. However, the increase for IL-6 and TNF-α correlated inversely with the level of Dgat1 mRNA in the cells, and a similar trend was observed for MCP-1. Thus, increased DGAT1 expression in BMD-Mϕ correlated with decreased secretion of proinflammatory substances in response to palmitate treatment.

The effects of DGAT1 expression on macrophage activation were specific for the M1 pathway. The mRNA levels of M2 pathway genes were generally more variable than those of the M1 markers (Supplemental Figure 2). Palmitate treatment did not induce their expression and, in fact, reduced mRNA levels of mannose receptor (Mrc2) in BMD-Mϕ of all genotypes. Moreover, the level of DGAT1 expression in these macrophages had no effect on the levels of M2 markers (Supplemental Figure 2).

Interestingly, the effects of increased DGAT1 expression in BMD-Mϕ were not restricted to M1 activation by FAs. Treatment combining the TLR4 ligand LPS, a canonical M1 stimulator, and IFN-γ also increased the mRNA expression of M1 genes in a manner that, in general, correlated inversely with Dgat1 mRNA levels (Supplemental Figure 3). In contrast, the level of DGAT1 expression did not affect the induction of M2 gene expression by treatment with the canonical M2 stimulator IL-4, with the exception of Mrc2, in which the effects of IL-4 were mitigated by increased DGAT1 expression (Supplemental Figure 3).

Because the M1 response was reduced in aP2-Dgat1 BMD-Mϕ treated with either palmitate or LPS/IFN-γ, we assessed whether the M1 activation potential of these cells was generally impaired. We treated WT and aP2-Dgat1 BMD-Mϕ with acetylated LDL (AcLDL) and nonopsonized yeast cell-wall β-glucan (zymosan) particles, which bind to scavenger receptors (44) and dectin-1 (45), respectively, and stimulate M1 macrophage activation. The mRNA levels of M1 genes in WT and aP2-Dgat1 BMD-Mϕ were similarly increased by either treatment (Supplemental Figure 4, A and B). Additionally, the phagocytic capacity of aP2-Dgat1 BMD-Mϕ activated by zymosan treatment was similar to that of WT cells (Supplemental Figure 4C). Collectively, these results indicate that the M1 activation capacity of aP2-Dgat1 macrophages is intact in response to other stimuli. We also assessed the M1 activation potential of aP2-Dgat1 macrophages in vivo by inducing peritonitis with thioglycollate treatment. After 3 days, the concentration of F4/80-positive P-Mϕ in the peritoneal fluid was similar in WT and aP2-Dgat1 mice (Supplemental Figure 4D), indicating normal macrophage recruitment, and the mRNA levels of M1 genes were similar in these cells (Supplemental Figure 4E). The mRNA levels of M1 genes were nearly undetectable in peritoneal cells from WT or aP2-Dgat1 mice treated with saline (control). These results indicate that the reduced WAT inflammation seen in aP2-Dgt1 and Tg→WT mice fed a high-fat diet is not due to a general defect in macrophage recruitment or activation potential.

Dgat1 mRNA levels in BMD-Mϕ are increased by PPARγ activation, and DGAT1 is required for PPARγ-mediated inhibition of palmitate-stimulated M1 activation. PPARγ agonists are potent antidiabetic agents that can suppress the M1 activation of cultured macrophages by palmitate treatment (13). Additionally, DGAT1 expression is increased by PPARγ agonist treatment in WAT and in cultured adipocytes (28–30). By extrapolation, we sought to determine whether PPARγ agonists regulate DGAT1 expression in macrophages and whether DGAT1 plays a role in PPARγ-mediated inhibition of M1 activation. Treatment of WT BMD-Mϕ with the PPARγ agonists pioglitazone (10 μM) or troglitazone (10 or 100 μM) increased Dgat1 mRNA levels approximately 2-fold, whereas treatment with 10 μM WY14643, a PPARα agonist, had no effect (Figure 9A). We next treated WT or Dgat1–/– BMD-Mϕ with either palmitate (150 μM) alone for 24 hours or with pioglitazone (10 μM) for 24 hours followed by palmitate and pioglitazone together for another 24 hours. As expected, the mRNA levels of M1 genes were increased by palmitate treatment, and this effect was inhibited by pre- and cotreatment with pioglitazone (Figure 9B). In contrast, pioglitazone treatment was unable to suppress the M1 activation in Dgat1–/– BMD-Mϕ (Figure 9B). A similar pattern was found for MCP-1, IL-6, and TNF-α levels in the secreted medium; these levels were increased by palmitate treatment and reduced by PPARγ agonists in WT cells, but the pioglitazone effect was absent in Dgat1–/– cells (Figure 9C). These data indicate that DGAT1 is required for the protective effects of pioglitazone in suppressing the M1 response of macrophages treated with saturated FAs.

Discussion

We demonstrate here that increased expression of the TG synthesis gene Dgat1 in macrophages is sufficient to protect against the inflammatory and metabolic consequences of DIO in vivo and against M1 inflammatory activation of macrophages treated with FAs or cytokines in vitro. aP2-Dgat1 transgenic mice, which had increased Dgat1 mRNA levels in the adipocyte/macrophage compartment, were prone to DIO but protected against DIO-associated nonadipose tissue steatosis, WAT and systemic inflammation, and insulin resistance. Remarkably, the protection against diet-induced WAT inflammation and insulin resistance in aP2-Dgat1 mice could be conferred to WT mice by the simple transfer of hematopoietic cells with increased DGAT1 expression, highlighting the importance of this enzyme within the macrophage compartment in preventing inflammation associated with excess lipids. In corroboration, in vitro studies of macrophages showed that Dgat1 mRNA levels correlated directly with macrophage TG storage capacity and inversely and specifically with M1 macrophage activation by palmitate. Further, Dgat1 mRNA levels in macrophages were regulated by PPARγ activation, and DGAT1 was required for PPARγ inhibition of the M1 response to palmitate treatment. These findings identify DGAT1 as an important modulator of lipid-induced inflammation in macrophages.

A finding of this study that we believe to be novel is that DGAT1 overexpression in the adipocyte/macrophage compartment of transgenic mice increased their propensity to DIO but markedly protected them from the associated deleterious metabolic and inflammatory consequences. In a prior study of the same aP2-Dgat1 mice, we showed that the aP2-Dgat1 transgene was expressed in the WAT and found that these mice were prone to DIO on a short-term (4 weeks) high-fat diet (24). In that study, we showed that glucose tolerance was similar in WT and aP2-Dgat1 mice in response to this short-term diet. In the current study, we show that these mice are protected from developing insulin resistance in response to a chronically high-fat diet (16 weeks). Moreover, this protection extended to include pronounced reductions in M1-type inflammation in the WAT and nonadipose tissue steatosis. The mRNA levels of several M1 inflammatory genes, including Ccl2, which encodes the macrophage-secreted chemokine MCP-1, and Tnfa, which encodes the inflammatory cytokine TNF-α, were decreased in the WAT of aP2-Dgat1 mice, and levels of inflammatory cytokines were lower in the circulation of aP2-Dgat1 mice with DIO. By crossing these mice with Adipoq–/– mice, we showed that this phenotype was not dependent on the presence of adiponectin, a hormone that is secreted by adipocytes and promotes insulin sensitivity (29, 37–40), thus suggesting alternative mechanisms, such as macrophage expression of the transgene.

A second major finding of this study is that increasing DGAT1 expression in macrophages by the transfer of hematopoietic cells was sufficient to protect mice from the deleterious consequences of DIO. Remarkably, BM transplantation of hematopoietic cells was sufficient to recapitulate the enhanced glucose metabolism and antiinflammatory aspects of aP2-Dgat1 mice. On the other hand, increasing DGAT1 expression in macrophages was insufficient to alter body weight or prevent diet-induced hepatic or skeletal muscle steatosis, indicating that the effects were specific for the insulin-sensitizing and antiinflammatory components of the aP2-Dgat1 phenotype and did not apply to TG partitioning. Of note, that Tg→WT mice experienced metabolic protection without a relative reduction in liver TG suggests that hepatic steatosis per se is unlikely to contribute significantly to the development of insulin resistance in this model.

Our findings in the BM transplantation studies do not discount the possibility that increased TG storage capacity in adipocytes may also contribute to the phenotype of aP2-Dgat1 mice. Indeed, enhanced capacity for FA storage in adipocytes may serve to limit the exposure of macrophages to proinflammatory FAs. Additionally, recent studies have shown that adipocytes can regulate macrophage activity (14, 46, 47). Studies focusing on adipocyte-specific DGAT1 expression in regulating the inflammatory and metabolic consequences of DIO are needed to address this question.

The phenotype in our 2 studies of aP2-Dgat1 mice contrasts with a report of a different aP2-Dgat1 transgenic line that exhibited glucose intolerance and tissue steatosis in response to a high-fat diet (48). While we do not know for certain what accounts for this discrepancy, our current study suggests that one possible contributing variable might be the amount of DGAT1 expression in macrophages, which was not measured in the other model. If those mice, in contrast to ours, have little aP2-driven DGAT1 expression in macrophages, then they may have been more prone to WAT inflammation and insulin resistance in response to a high-fat diet. Other variables that may contribute to the different phenotypes include genetic background (the other model was on an FVB background, whereas our model was on C57BL/6) or the timing or duration of the high-fat diet employed. The other mice were studied after 6 weeks of a high-fat diet starting at the age of 24–29 weeks, whereas we studied the effects of high-fat diets of at least 16 weeks starting at age 12 weeks.

Our BM transplantation studies suggested that macrophages with increased DGAT1 and increased lipid synthesis capacity might be protected from the proinflammatory effects of lipids. Indeed, we found that macrophages isolated from mice that overexpress DGAT1 had an increased capacity for TG storage and were resistant to the M1 inflammatory response that results from treatment with palmitate. Conversely, macrophages lacking DGAT1 were more sensitive to palmitate-stimulated M1 activation. These findings are consistent with DGAT1 having a role in protecting cells from lipotoxicity mediated by FAs, as was shown in other cell types (27). In the case of macrophages within the WAT, this function for DGAT1 may be of considerable importance, since these cells may encounter and take up large amounts of lipids by endocytic or phagocytic means.

Precisely how DGAT1 protects against M1 macrophage activation by FAs is unclear. We found that Dgat1 mRNA levels correlated inversely with the level of M1 activation in macrophages treated with palmitate or the combination of LPS (a TLR4 ligand) and IFN-γ. Interestingly, this correlation was not seen when M1 activation was stimulated in WT and aP2-Dgat1 macrophages by treatment with AcLDL, a ligand for scavenger receptors (44), or nonopsonized zymosan, a ligand for dectin-1 (45). Taken together, these findings suggest that palmitate and LPS/IFN-γ may signal through a shared downstream step modulated by DGAT1. This finding is consistent with other work suggesting that saturated FAs and LPS engage common signaling elements, including JNK1, JNK2, NF-κB, and activating transcription factor 3, an NF-κB target (13–17, 49).

FAs may also regulate macrophage activation by mechanisms distinct from that of LPS. In support of this, the kinetics by which LPS treatment upregulates Tnfa mRNA levels in RAW 264.7 macrophages were quite different from those induced by palmitate treatment (14). While LPS acts extracellularly, our findings support DGAT1 functioning to modulate FA flux intracellularly. Increased esterification of intracellular FAs into the TG pool may act as a “sink” to lower their flux into pathways affecting the levels of signaling metabolites linked to inflammation (ceramides, eicosanoids, diacylglycerols, lysophosphatidic acids) and ER stress, which itself can induce JNK phosphorylation and NF-κB activation in cells (20–22, 50–53).

In contrast to the effects on the M1 pathway, the level of Dgat1 mRNA expression in macrophages had little effect on IL-4–mediated activation of the M2 response, further highlighting the specificity of the DGAT1 effect on inflammatory pathways. We note, however, that a more appropriate analysis of the consequences of altering DGAT1 expression on the M2 pathway in macrophages would require studying mice on the BALB/c genetic background, which exhibit a more robust M2 macrophage phenotype than do those on the C57BL/6 background in the current study (54).

By sensing levels of intracellular FA metabolites, PPARγ links nutritional status to the transcriptional regulation of metabolic genes. In macrophages, PPARγ activity regulates the expression of M1 and M2 genes (19, 31–33, 55) and modulates FA-induced inflammatory activation (13). Since PPARγ activation increases Dgat1 mRNA levels in adipocytes (28–30), we hypothesized that a similar pathway may exist in macrophages. Indeed, mRNA levels of Dgat1 were increased by pharmacologic activation of PPARγ in cultured macrophages. More importantly, DGAT1 was required for the antiinflammatory effects of PPARγ in suppressing FA-mediated M1 inflammatory activation. This suggests that DGAT1 is an important mediator of the beneficial effects of PPARγ agonists in this cell type. Chronic DIO in humans, as in mice, is associated with WAT inflammation (5), and the systemic manifestation of this inflammation is ameliorated by treatment with PPARγ agonists (33). Our findings suggest that the level of DGAT1 expression in human macrophages is a determinant of this process and that DGAT1 may be involved in the antiinflammatory effects of PPARγ.

We note that the mRNA levels of both murine Dgat1 and Dgat2 were markedly increased in WT P-Mϕ in response to chronic high-fat feeding. This pattern likely reflects an adaptive change in the gene expression program of macrophages to facilitate the esterification of high levels of FAs and their derivatives. The mechanism for these changes in DGAT gene expression in macrophages is unknown but offers an opportunity for further investigation.

The current findings raise an interesting paradox when compared with those from DGAT1-knockout mice, which also exhibit increased insulin sensitivity (56) and reduced markers of inflammation in the WAT (R. Streeper, S. Cases, and R. Farese, unpublished observations). Thus, whole-body DGAT1 deficiency is associated with reduced WAT inflammation, yet DGAT1 deficiency in isolated macrophages increased the propensity to FA-mediated inflammation. What could account for this? We suspect that whole-body DGAT1 deficiency effectively prevents FA accumulation in the WAT, through shunting of FA to oxidative and thermogenic pathways and through a decreased rate at which dietary FAs enter the circulation (57). In such a model, DGAT1-deficient macrophages would not be exposed to toxic levels of FAs that would normally induce inflammation. Thus, the overall phenotypic effects of DGAT1 deficiency may depend on the relative contributions of different cell types. This implication may have clinical relevance, since highly potent and specific inhibitors of DGAT1 activity are being developed to treat clinical obesity and related TG-associated disease (58).

Methods

Mice. Studies were of WT C57BL/6J and genetically modified mice, including aP2-Dgat1 transgenic (24), Dgat1–/– (56), and Adipoq–/– mice (39). aP2-Dgat1, Dgat1–/–, and Adipoq–/– mice were on a C57BL/6J background (backcrossed for more than 10 generations). Pups were weaned onto a standard 5053 PicoLab chow diet (Purina). For DIO studies, 12-week-old mice were fed a Western-type diet containing 20% anhydrous milk fat, 1% corn oil, and 0.2% cholesterol by weight (TD.01064; Harlan-Teklad) for 16 weeks. For BM transplantations, donor mice were C57BL/6J (CD45.2; Jackson Laboratory), and recipients were B6.SJL-PtprcaPep3b/BoyJ (CD45.1; Taconic). Anesthesia was induced with isoflurane (survival procedures) or with avertin or halothane (terminal procedures). All procedures were approved by the UCSF Animal Research Committee and followed NIH guidelines.

Isolation of BMD-Mϕ. Marrow from the femurs and tibias of 22- to 26-week-old mice fed a chow or a chronic high-fat diet was collected by flushing with 10 ml of RPMI (Gibco; Invitrogen) containing 20% heat-inactivated FBS (Hyclone). The suspension was passed through a 70-μm cell strainer, incubated in red cell lysis buffer for 10 minutes at room temperature, washed twice, and resuspended in RPMI with FBS. Cells were plated at a density of 1 to 2 × 106 per well in medium supplemented with 30% L929-conditioned medium to stimulate differentiation of precursors into BMD-Mϕ. Noncoated tissue culture plates were used to prevent adherence of dendritic and nonprogenitor cells. The medium was changed every 3 days; after 6 days, nearly all cells had differentiated into macrophages by visual analysis. Cells were harvested 8 to 12 days after plating.

Isolation of primary P-Mϕ. The peritoneal cavities of mice fed a chow or chronic high-fat diet were infused with 10 ml of ice-cold PBS, and after agitation, approximately 7 ml of fluid recovered from each mouse was processed and plated as described for BM samples. Cells were washed 3 hours after plating to isolate adherent P-Mϕ and cultured for 3 days, after which the medium was changed. P-Mϕ were used 4 days after plating.

BM transplantation. To facilitate the assessment of BM reconstitution, the genetic background of the recipient mice (B6.SJL-Ptprca Pep3b/BoyJ) was identical to that of the donor mice (C57BL/6), except for a single point mutation in the leukocyte antigen Ptprc (CD45.2). The mutant version of Ptprc (CD45.1) is functionally equivalent, but allows the identification of cells that are of recipient (CD45.1) or donor (CD45.2) origin in peripheral blood leukocytes by FACS (see below). BM cells harvested from 8-week-old WT or aP2-Dgat1 donor mice were resuspended in PBS with 0.1% FA-free BSA, and 1 to 1.2 × 106 donor cells were injected into age- and sex-matched recipient mice by tail vein. Recipient mice were irradiated in two 5-Gy doses spaced 3 hours apart 1 day before injection. After BM injections, recipient mice were placed in their home cages with antibiotic water for 1 month, after which blood was drawn for analysis of BM reconstitution by FACS and for detection of aP2-Dgat1 leukocytes with transgene-specific primers. The mice then recovered under usual care until they were 12 weeks old, at which time they were placed on a high-fat diet. Glucose tolerance tests (GTTs) and insulin tolerance tests (ITTs) were performed as for other cohorts of mice after 16 weeks of diet, and tissues were harvested after 20 weeks of diet.

FACS analyses. The percentage of CD45.1+ (recipient) and CD45.2+ (donor) cells in the peripheral blood of BM-transplanted mice was determined by flow cytometry (FACSCalibur; BD Biosciences). Data were acquired with CellQuest Pro software (version 5.1.1; BD Biosciences) and analyzed using FlowJo software (version 6.4.7; Tree Star). Gating was set using the Zebra plot feature of FlowJo, based on unstained samples, and CD45.1+ and CD45.2+ cells were identified using FITC-coupled anti-CD45.1 (1:200) and allophycocyanin-coupled (APC-coupled) anti-CD45.2 (1:1000) antibodies, respectively (BD — Pharmingen). The percentage of donor cells was expressed by multiplying the total number of live cells by the percentage of CD45.2+ cells.

To measure acute macrophage recruitment, peritoneal fluid was obtained from mice 3 days after intraperitoneal injection with 1 ml of 1% thioglycollate (BD Biosciences) to induce transient aseptic peritonitis. The percentage of macrophages in this fluid was determined by flow cytometry as above, and macrophages were identified using a PE-conjugated anti-F4/80 antibody (1:1000; Caltag Laboratories). The concentration of P-Mϕ was expressed by multiplying the total number of live cells in the peritoneal fluid by the percentage of F4/80+ cells.

Separation of SVF and adipocyte fractions of WAT. Epididymal fat pads were excised from adult chow-fed mice and placed in HBSS (Gibco; Invitrogen) containing 1% HEPES and 3% BSA. Fat pads were finely minced, washed twice in DMEM/F-12 (Gibco; Invitrogen), and placed in DMEM/F-12 containing 1 mg/ml collagenase (type I; Worthington) at 37°C for 30 minutes with gentle agitation. The cell suspension was filtered through a 250-μm nylon filter (Nitex; Safar America), and the filtrate was spun at 80 g for 5 minutes at room temperature to separate the pellet containing the SVF from the floating adipocytes. The adipocytes were resuspended in medium containing 5 mM EDTA and 2% BSA in PBS and spun again at 200 g for 5 minutes. Floating cells were plated. SVF cells were spun again at 600 g, and the pelleted cells were plated as for PM-ϕ.

Real-time PCR. RNA was isolated using RNA Stat-60 (Tel-Test), according to the manufacturer’s protocol, from homogenized whole epididymal WAT, separated WAT fractions, or cultured macrophages. RNA (0.5–2 μg) was reverse-transcribed with SuperScript III reverse transcriptase and random hexamers (Invitrogen) to generate cDNA. Real-time qPCR was performed with an ABI Prism 7700 (Applied Biosystems) and SYBR green detection of amplified products. Each 25-μl PCR reaction mix contained 2 μl of cDNA, 12.5 μl of SYBR green master mix (QIAGEN), and 10 pmol of each primer. Relative mRNA abundance was normalized to the internal standard cyclophilin with the ΔΔCT method, as described by the manufacturer (Invitrogen). Primer sequences are listed in Supplemental Table 1.

Immunoblotting. The abundance of DGAT1 protein was detected in BMD-Mϕ by immunoblotting. Briefly, confluent cells in 6-well plates were partially dislodged by incubating them at 37°C in PBS with 10 mM EDTA for 10 minutes. The cells were then washed twice, manually scraped into 200 μl of PBS, and spun at 800 g for 5 minutes. The supernatant was discarded, and the cells were resuspended in 500 μl of buffer containing 50 mM Tris (pH 7.4) and 250 mM sucrose. The suspended cells were passed several times through a 27-gauge needle, then spun at 15,000 g (max) for 5 minutes at 4°C. Protein (10 μg) from the supernatant of each sample was loaded onto a 10% Bis-Tris gel (NuPAGE; Invitrogen), and SDS-PAGE was performed using compound 3-(N-morpholino) propanesulfonic acid (MOPS) as the running buffer. Proteins were transferred to PVDF membranes over 90 minutes, and membranes were blocked at 4°C overnight in 0.1% Tween-20 containing 5% nonfat milk (TBS-T). Membranes were then washed and incubated in TBS-T containing 1:2000 anti-DGAT1 antibody (polyclonal rabbit anti-mouse) for 2 hours, washed again, and incubated for another 2 hours in TBS-T containing 1:2000 HRP-conjugated anti-rabbit IgG (ECL; GE Healthcare). Protein abundance was detected by chemiluminescence (ECL-plus). As an internal loading control, membranes were stripped and reprobed with murine monoclonal anti–β-actin antibody (1:2500; Sigma-Aldrich) for 45 minutes and incubated in TBS-T containing HRP-conjugated anti-mouse IgG for 1 hour prior to detection of chemiluminescence (Super Signal West Pico; Thermo Scientific).

Measurement of tissue TG content. Liver and skeletal muscle (gastrocnemius and soleus) samples were pulverized in liquid nitrogen and homogenized in buffer A (50 mM Tris-HCl, pH 7.4, 250 mM sucrose) containing proteinase inhibitors. Lipids were extracted in chloroform:methanol (2:1) and separated by TLC on silica gel G-60 plates with the solvent hexane:ethyl ether:acetic acid (80:20:1). The TG bands were visualized by exposure to iodine and then scraped and analyzed as described (59), with triolein (Sigma-Aldrich) as a standard, and expressed per tissue weight.

Measuring incorporation of FAs into cellular TG. FA fluxes were followed in BMD-Mϕ treated with medium containing oleate or palmitate. Each FA was a mixture of cold (100 μM) and 14C-labeled (0.04 μCi/ml) forms, with the label appearing at the distal carbon. Cells were incubated for 24 hours, after which total lipid was extracted from cell lysates and separated by TLC to visualize the TG fraction as above. FA incorporation was then determined by scintillation counting of 14C from both total cellular lipid and the cellular TG fraction, respectively.

Nile Red fluorescence assay. BMD-Mϕ cultured in 12-well plates (BD Falcon) were incubated in DMEM plus FBS alone or in medium containing either 200 μM oleate or 150 μM palmitate (both from Sigma-Aldrich). Oleate and palmitate were prepared and complexed with BSA (2:1 molar ratio of FA to albumin) as described (27). After 24 hours, intracellular neutral lipid content was measured by Nile Red fluorescence with the AdipoRed assay reagent as described by the manufacturer (Cambrex). Fluorescence was measured with a Victor3 1420 fluorometer (PerkinElmer) at excitation and emission wavelengths of 485 nm and 572 nm, respectively. To correct for nonspecific fluorescence, measurements taken before incubation with Nile Red were subtracted from those taken after incubation.

Activation of M1 and M2 inflammatory pathways in BMD-Mϕ. Cells were incubated in medium alone (control), for 24 hours in medium containing either 150 μM palmitate, 100 U/ml IFN-γ plus 5 ng/ml LPS, or 10 ng/ml IL-4 (all from Sigma-Aldrich), for 6 hours in medium containing 50 μg/ml AcLDL (gift from Tobias Walther, Max Planck Institute of Biochemistry, Martinsried, Germany), or for 2 hours in medium containing zymosan at a particles/cells ratio of approximately 50:1 (Cell BioLabs). Cells were then lysed for RNA isolation, and the medium was collected for cytokine measurements. The concentration and duration of palmitate treatment have been shown to be nontoxic (12), and we did not observe any signs of toxicity in the cells we treated. Activation of PPARγ in BMD-Mϕ was stimulated by incubating cells with troglitazone (Sigma-Aldrich) or pioglitazone (gift from Brian Hubbard). Activation of PPARα was stimulated by incubating cells with WY14643 (Sigma-Aldrich).

Phagocytosis assay. Phagocytosis of zymosan particles by BM-Mϕ was measured colorimetrically at 405 nm using a kit (Cell BioLabs) per manufacturer instructions.

Immunohistochemistry. Formalin-fixed, paraffin-embedded epididymal WAT sections were deparaffinized, rehydrated, and treated with antigen-unmasking reagent, as described by the manufacturer (Vector Laboratories). Sections were blocked in normal serum and incubated with biotinylated anti-F4/80 antibody (Serotec) overnight. Endogenous HRP activity was quenched by incubation with 3% hydrogen peroxide for 10 minutes. Samples were then incubated with streptavidin-HRP (BD Biosciences), and specific HRP activity was detected with 3,3′-diaminobenzidine (DAB; Vector Laboratories). Sections were counterstained with hematoxylin before dehydration and mounting. CLS were counted from 10 separate ×20 fields per sample in serial samples, and the mean numbers of CLS per sample in each group were plotted.

Analyses of serum and medium. Mice were fasted for 12 hours (overnight) for lipid analyses and 8 hours for hormone levels. Blood was obtained from tail veins of unanesthetized mice, and kits were used to measure the levels of free FA (Wako Pure Chemical Industries), TG (Roche Diagnostics), and total cholesterol (Wako). Levels of insulin, adiponectin, and resistin in serum and levels of inflammatory markers (MCP-1, IL-6, PAI-1, and TNF-α) in both serum and culture medium were measured by multiplexed bead-based immunoassays (Millipore Corporation) using xMAP technology (Luminex). Blood glucose of mice fasted for 8 hours was measured with a glucometer (OneTouch Ultra; LifeScan).

Assessment of glucose and insulin tolerance and insulin sensitivity in vivo. Glucose tolerance was assessed in mice after an 8-hour fast by measuring basal blood glucose and monitoring glucose excursion 15, 30, 60, 90, and 120 minutes after a peritoneal injection of dextrose (1 g/kg). Insulin tolerance was assessed in mice after a 2-hour fast by measuring basal blood glucose and its excursion after an injection of insulin (1 U/kg). Insulin sensitivity was expressed as an index (HOMA-IR) calculated as follows: (G0 × I0)/22.5, where G0 is fasting glucose (mmol/l), and I0 is insulin (μU/ml) (60).

Statistics. Data are presented as the mean ± SEM. Measurements were compared by 2-tailed Student’s t test or Mann-Whitney rank-sum test. Body weights were compared by repeated-measures ANOVA with Bonferroni’s post-hoc analysis. GTTs and ITTs were analyzed similarly and also by comparing the areas under each curve calculated by the trapezoid rule (Prism4; GraphPad Software). Significance was determined at P < 0.05.

Supplemental data

Acknowledgments

We thank S. Coughlin for facilitating BM transplantation experiments, C. Mrejen for assistance with TLC analyses in macrophages, Y. Si for assistance with FACS of blood samples, K. Veenstra and S. Marmor for performing immunoassays, J.D. Fish for histological assistance, R. Bituin for mouse husbandry, G. Howard for editorial assistance, D. Jones for manuscript preparation, and members of the Farese laboratory for discussions and comments. This work was supported by grants from the NIH (DK-056084 to R.V. Farese Jr.; DK08174-01 to S.K. Koliwad; animal facilities grant NIH/NCRR CO6 RR018928; and the UCSF Diabetes, Endocrinology and Metabolism Training Grant NIDDK DK07418-27 to S.K. Koliwad) and the A.P. Giannini Foundation for Medical Research (to S.K. Koliwad), and by the J. David Gladstone Institutes.

Footnotes

Conflict of interest: The authors have declared that no conflict of interest exists.

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